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Revision as of 12:18, 29 September 2013 (view source) Biru (Talk | contribs) (Created page with "{ "date":"2013-07-03", "author":"viola", "title":"<html>cloning of the terminators with EFE</html>", "content":"<html> <a href=\"https://2013.igem.org/wiki/index.php?title=Team:UN...") ← Older edit		Latest revision as of 10:49, 3 October 2013 (view source) Ggirelli (Talk | contribs)
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-	{	+	{"date" : "2013-07-31","author" : "thomas","title" : "pSpac + GFP cloning!!!","content" : "<html>Today I started a new cloning in order to obtain GFP in the vector pSBBs0K-Pspac (<a href=\"http://parts.igem.org/Part:BBa_K823026\">BBa_K823026</a>). This construct will be useful to Emil in order to characterize Pspac at difference concentration of inducer (IPTG). I started performing a PCR on the GFP following the <a href=\"https://2013.igem.org/Team:UNITN-Trento/Protocols#Phusion-PCR\">Phusion PCR protocol</a>. I used BB_fwd and BB_rev primers to obtain an amplification of the insert. This because the GFP backbone (<a href=\"http://parts.igem.org/partsdb/get_part.cgi?part=BBa_E0840\">BBa_E0840</a>) had the same antibiotic resisistance of our destination vector BBa_K823026 (Amp). I obtain a PCR product with a concentration of 146 ng/&micro;l, confirmed by electrophoresis analysis.</html>{{:Team:UNITN-Trento/Templates/Styles/Spoiler|Gel image|<html><center><img src=\"https://static.igem.org/mediawiki/2013/5/5c/Tn-2013_gel_E0840_PCR.jpg\" width=\"450px\" /></center></html>}}<html>  I continued then with the restriction digestions following <a href=\"https://2013.igem.org/Team:UNITN-Trento/Protocols#Digestion\">this protocol</a>. I digested BBa_K823026 using SpeI and PstI, and PCR product with XbaI and PstI. <br/>The two digestion products were then purified and quantified: GFP PCR 60 ng/&micro;l, BBa_K823026 19 ng/&micro;l. The last step was then the ligation that was performed following <a href=\"https://2013.igem.org/Team:UNITN-Trento/Protocols#Ligation\">this protocol</a>. The ligation products were then plated on CM plates. </html>","tags" : "pSpac-GFP"}
-	"date":"2013-07-03",	+
-	"author":"viola",	+
-	"title":"<html>cloning of the terminators with EFE</html>",	+
-	"content":"<html> <a href=\"https://2013.igem.org/wiki/index.php?title=Team:UNITN-Trento/Notebook#tn-post-2013-07-02-viola\">Yesterday's ligation</a> seemed to work and and this evening i'll make some inocula... </html>",	+
-	"tags":"EFE"	+
-	}	+

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Latest revision as of 10:49, 3 October 2013

{"date" : "2013-07-31","author" : "thomas","title" : "pSpac + GFP cloning!!!","content" : "Today I started a new cloning in order to obtain GFP in the vector pSBBs0K-Pspac (BBa_K823026). This construct will be useful to Emil in order to characterize Pspac at difference concentration of inducer (IPTG). I started performing a PCR on the GFP following the Phusion PCR protocol. I used BB_fwd and BB_rev primers to obtain an amplification of the insert. This because the GFP backbone (BBa_E0840) had the same antibiotic resisistance of our destination vector BBa_K823026 (Amp). I obtain a PCR product with a concentration of 146 ng/µl, confirmed by electrophoresis analysis.

I continued then with the restriction digestions following this protocol. I digested BBa_K823026 using SpeI and PstI, and PCR product with XbaI and PstI.
The two digestion products were then purified and quantified: GFP PCR 60 ng/µl, BBa_K823026 19 ng/µl. The last step was then the ligation that was performed following this protocol. The ligation products were then plated on CM plates. ","tags" : "pSpac-GFP"}